Rather, it is more likely that the treatment failed to effectively neutralize the relatively higher amount of TNF in A/J mice. Future studies will be required to assess the extent to which TNF drives pregnancy
loss in A/J mice and the pathogenic pathways activated by this cytokine in both strains. Current evidence implicates the inflammation–coagulation cycle as a central mediator for malaria-induced pregnancy compromise in B6 mice (21) (Avery et al., manuscript submitted). However, it is known that inflammatory cytokines like TNF are directly embryotoxic (44), inducing trophoblast apoptosis via TNF receptors (45), especially if the cytokine is released by monocytes in direct contact with trophoblast (46). A potential role for apoptosis in the pathogenesis
of placental malaria is currently being GSK-3 assay assessed in both mouse strains. In the context of high levels of high pro-inflammatory cytokines, IL-10 plays a regulatory role (7,47), blocking malaria-associated immunopathology and P. chabaudi virulence (48). In this study, as pro-inflammatory cytokine levels increased in infected pregnant A/J mice, regulatory IL-10 decreased, at experiment day 10 reaching levels significantly lower than in infected pregnant B6 mice. While elevated IL-10 may serve to partially dampen inflammatory damage in P. chabaudi AS-infected pregnant selleckchem mice (20), it is inadequate to prevent pregnancy loss in both A/J and B6 mice. In humans, this cytokine level is significantly higher in infected primigravidae compared with their uninfected counterparts and has been proposed to be a marker Oxymatrine for inflammatory placental malaria (49). Elevated levels of sTNFRII, which can serve to bind and sequester TNF, are likewise apparently inadequate to
control TNF-mediated pathogenesis; however, the specific role played by this solubilized receptor in infected mice and women with placental malaria (49,50) remains to be established. The different dynamics of cytokine expression in infected A/J and B6 mice prompted an examination of the potential cell types that may contribute to these differences at the splenic level. In general, lymphocyte and myeloid cell levels were influenced only by infection status, with strain and pregnancy having no significant impact, although only infected pregnant B6 mice show early elevation of neutrophils and monocytes (at experiment day 9). Interestingly, however, 1 day later, infected pregnant A/J mice showed elevated monocyte and inflammatory monocyte levels relative to uninfected pregnant mice. While these observations clearly demonstrate that pregnancy does not alter infection-induced splenic cellular expansion in either strains, they do not shed any light on the differential dynamics of embryo loss in A/J and B6 mice.